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首页> 外文期刊>Clinical Chemistry: Journal of the American Association for Clinical Chemists >Rapid method for eliminating labile glycosylated hemoglobin from the assay for hemoglobin A1.
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Rapid method for eliminating labile glycosylated hemoglobin from the assay for hemoglobin A1.

机译:从血红蛋白A1分析中消除不稳定的糖基化血红蛋白的快速方法。

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摘要

The irreversible formation of stable glycosylated hemoglobin proceeds through a labile intermediate that is indistinguishable, by most methods, from the stable glycosylated product. The inclusion of the labile intermediate, which changes acutely with acute blood glucose changes, detracts from the utility of the assay as an index of chronic glucose concentration. We have developed a rapid, reliable chemical method for eliminating the labile intermediate: a 30-min incubation of whole-blood samples with semi-carbazide (30 mmol/L) and aniline (12 mmol/L) at pH 5 and 38 degrees C. The semicarbazide serves as a glucose trap; the transfer of glucose from the labile glycosylated hemoglobin to the semicarbazide is catalyzed by the acidic pH and aniline. This treatment is effective in the three most commonly used assays: "high-performance" liquid chromatography, electrophoresis, and a minicolumn kit.
机译:稳定的糖基化血红蛋白的不可逆形成是通过不稳定的中间体进行的,该中间体在大多数方法中都与稳定的糖基化产物没有区别。不稳定的中间体的含量随急性血糖的变化而急剧变化,这不利于测定作为慢性葡萄糖浓度的指标的实用性。我们已开发出一种快速,可靠的化学方法来消除不稳定的中间体:在pH 5和38摄氏度下,将半血肼(30 mmol / L)和苯胺(12 mmol / L)的全血样品孵育30分钟氨基脲用作葡萄糖阱;酸性pH值和苯胺催化葡萄糖从不稳定的糖基化血红蛋白向氨基脲的转移。这种处理在三种最常用的测定中有效:“高效”液相色谱,电泳和微型柱试剂盒。

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